Issue 1, 2014

Ratiometric fluorescence imaging of lysosomal Zn2+ release under oxidative stress in neural stem cells

Abstract

Zinc dyshomeostasis is a major mechanism of neuronal death, which is involved in many different neuropathological conditions. Lysosomal membrane permeabilisation has an important function in zinc-induced neuronal death under oxidative stress. To investigate lysosomal zinc functions in neurons with high spatial and temporal reliability, we report a ratiometric probe, LysoZn-1. It is derived from the styryl-BODIPY-DPA scaffold with a lysosome-targeted 2-morpholinoethylamine moiety to allow localisation in lysosomes. The electron donor at the meso-position of the BODIPY fluorophore makes the present probe prefer complexing with Zn2+ rather than Cd2+, which can be explained by HSAB (Hard–Soft Acid–Base) theory and was confirmed by Gaussian calculation. Upon Zn2+ binding, LysoZn-1 exhibits obvious fluorescence enhancement (F578 nm) and ratio (F578 nm/F680 nm) changes. The emission intensities of LysoZn-1 and LysoZn-1 + Zn2+ do not change significantly under lysosomal pH ranging from 4.5 to 6.0. Confocal imaging experiments indicate that LysoZn-1 is able to localise to lysosomes in neural stem cells (NSCs), MCF-7 and Hela cells and detect exogenous Zn2+ levels in NSCs and MCF-7 cells. LysoZn-1 function is not disturbed by chloroquine in living cells. Furthermore, increases in lysosomal Zn2+ concentration upon H2O2 stimulation in NSCs are observed using LysoZn-1.

Graphical abstract: Ratiometric fluorescence imaging of lysosomal Zn2+ release under oxidative stress in neural stem cells

Supplementary files

Article information

Article type
Paper
Submitted
29 Jul 2013
Accepted
14 Aug 2013
First published
11 Sep 2013

Biomater. Sci., 2014,2, 89-97

Ratiometric fluorescence imaging of lysosomal Zn2+ release under oxidative stress in neural stem cells

H. Zhu, J. Fan, S. Zhang, J. Cao, K. Song, D. Ge, H. Dong, J. Wang and X. Peng, Biomater. Sci., 2014, 2, 89 DOI: 10.1039/C3BM60186B

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